Archiving of vectors

ABSTRACT

The invention relates to a solid medium or matrix for storage of nucleic acid molecules (e.g. RNA and/or DNA), particularly vectors and especially plasmids, comprising a solid matrix preferably having a compound or composition which protects against degradation of nucleic acids incorporated into or absorbed on the matrix. The invention also relates to methods for storage or isolation/purification of nucleic acids using this solid medium, and in situ use of the stored or isolated/purified nucleic acids.

CROSS REFERENCE TO RELATED APPLICATIONS

[0001] The present application claims the benefit of the filing dates of U.S. Application No. 60/093,073, filed Jul. 16, 1998, and No. 60/100,737, filed Sep. 17, 1998, the disclosures of which are incorporated by reference herein in their entireties.

BACKGROUND AND SUMMARY OF THE INVENTION

[0002] The present invention relates to a solid medium or support for use in the storage (preferably the long term storage) of nucleic acids (e.g. DNA and RNA, ribosomal RNA and messenger RNA), particularly one or more vectors and especially one or more plasmids, and to methods which comprise the use of this solid medium or support. In particular, the invention relates to a method for storage and transport of such nucleic acids or vectors on the solid medium, as well as to methods which involve either recovery or purification of the nucleic acids or vectors from the solid medium, or the use or manipulation of the nucleic acids or vectors obtained from or contained by or on the solid medium. Such use or manipulation includes, for example, digestion (e.g. with one or more nucleases, exonucleases or endonucleases such as restriction enzymes), synthesis (e.g. with one or more polymerases and/or reverse transcriptases), amplification (e.g. by polymerase chain reaction with one or more polymerases), sequencing (e.g. with one or more polymerases), or transformation or transfection into one or more host cells using, for example, chemically competent or electrocompetent cells or using known transfection reagents and techniques. The preferred medium or support is a matrix which protects against degradation of nucleic acid incorporated onto the matrix. Such a matrix may comprise an absorbent cellulose-based matrix or paper, or a micromesh of synthetic plastic material such as those described in U.S. Pat. No. 5,496,562, which is incorporated by reference herein. Preferably, the matrix comprises a composition comprising a weak base, a chelating agent, an anionic surfactant or anionic detergent, and optionally uric acid or a urate salt, wherein said composition is absorbed on or incorporated into said matrix. FTA™ paper and derivatives, variants and modifications thereof are included among such supports.

[0003] Another aspect of the invention relates to such a solid medium or support for use in the sampling, purifying and/or analyzing of one or more non-chromosomal DNA (e.g. mitochondria, chloroplast, F′) and to methods which comprise the use of this solid medium or support for such purposes.

[0004] For many projects, generation of numerous DNA samples from biological specimens is routine. Handling and archiving a large collection can become a logistical problem for the laboratory. One solution, used in forensic labs, is the blood-storage medium FTA™ Cards. An FTA™ Card stores genomic DNA in the form of dried spots of human whole blood, the cells of which were lysed on the paper. Stored at room temperature, genomic DNA on FTA™ paper is reported to be stable at least 7.5 years (Burgoyne, et al., Conventional DNA Collection and Processing: Disposable Toothbrushes and FTA™ Paper as a Non-threating Buccal-Cell Collection Kit Compatible with Automatable DNA Processing, 8^(th) International Symposium on Human Identification, Sep. 17-20, 1997). Before analysis of the captured DNA, a few simple washing steps remove the stabilizing chemicals and cellular inhibitors of enzymatic reactions. Since the DNA remains with the paper, the manipulations to purify the DNA are simplified and amenable to automation. DNA samples on FTA™ Cards offer a very compact archival system compared to glass vials or plastic tubes located in precious freezer space.

[0005] Bacterial DNAs spotted on FTA™ Cards may be an efficient system for storage and retrieval as well. Recently, Rogers and Burgoyne characterized by PCR-ribotyping culture samples of several bacterial strains of Staphylococcus and E. coli stored on FTA™ Cards (Rogers, et al., (1997) Anal. Biochem. 247:223). Further, purified plasmid DNA was efficiently recovered after spotting on treated paper, however, encasement of the paper in polystyrene was used for storage (Burgoyne, U.S. Pat. No. 5,496,562, which is incorporated by reference herein).

[0006] According to the present invention, any nucleic acids (e.g. RNA and DNA and particularly RNA and DNA vectors) may be archived and later recovered and/or manipulated by a simple and efficient method in which the host carrying the one or more nucleic acids or vectors are contacted with a solid medium (preferably FTA™ paper or derivatives, variants or modifications thereof), without the need to encase the support or use protective coatings (such as polystyrene) to store the nucleic acids or vectors. Thus, the invention avoids the need to use organic solvents or harsh chemicals to remove such protective coatings before use, manipulation, purification or isolation of the nucleic acid molecules or vectors can take place. In another aspect, purified nucleic acid molecules or vectors may be used, although in a preferred aspect, crude preparations (unpurified vector preparations) containing the one or more nucleic acid molecules or vectors may be contacted with the solid medium or support. Thus, the invention provides methods to isolate and/or purify nucleic acid molecules or vectors from any sample containing one or more vectors such as host cells, viruses, viral plaques, and/or crude preparations from biological materials (such as host cell or virus extracts, lysates, debri, hydrolysates, and the like). Such isolated and/or purified nucleic acid molecules or vectors obtained from or contained by the solid support or matrix may be used or manipulated in one or more standard molecular biology techniques, such as digestion, sequencing, amplification, synthesis and transformation/transfection reactions. In a particularly preferred aspect, one or more host cells containing the nucleic acid molecules or vectors to be isolated, stored and/or manipulated can be contacted directly with the medium or support. According to the present invention, host cell cultures or colonies from plates may be used. Preferred host cells for use in the invention include prokaryotic or eukaryotic host cells, particularly gram positive and gram negative bacteria such as Escherichia, Streptomyces, Pseudomonas, and the like.

[0007] Other preferred embodiments of the present invention will be apparent to one of ordinary skill in light of what is known in the art, in light of the following drawings and description of the invention, and in light of the claims.

BRIEF DESCRIPTION OF THE DRAWINGS

[0008]FIG. 1 is a PCR analysis of bacterial genomic DNA on an FTA™ Card. The agarose gel analysis of the amplification products pictured are shown as follows: lanes 1-3: Agrobacter tumefaciens strain LBA4404; lanes 4-6: Agrobacter tumefaciens strain EHA101; lanes 7-9: E. coli DH10B strain; lanes 10-12: Streptomyces coelicolor; lanes 13-15: S. lividans; and lanes 16-18: S. paralus. Molecular size standards are a Low DNA Mass™ Ladder (M1) and a 1 Kb DNA Ladder (M2).

[0009]FIG. 2 is a PCR analysis of plasmid DNA from E. coli (DH10B) on an FTA™ Card.

[0010]FIG. 3 is a PCR analysis of plasmid and genomic DNA from saccharomyces cerevisiae on an FTA™ Card.

DETAILED DESCRIPTION OF THE INVENTION

[0011] In the description that follows, a number of terms used in the fields of molecular biology and recombinant DNA technology are utilized extensively. In order to provide a clearer and consistent understanding of the specification and claims, including the scope to be given such terms, the following definitions are provided.

[0012] Amplification. As used herein, “amplification” refers to any in vitro method for increasing the number of copies of a nucleotide sequence with the use of a polymerase. Nucleic acid amplification results in the incorporation of nucleotides into a nucleic acid (e.g., DNA) molecule or primer thereby forming a new nucleic acid molecule complementary to the nucleic acid template. The formed nucleic acid molecule and its template can be used as templates to synthesize additional nucleic acid molecules. As used herein, one amplification reaction may consist of many rounds of nucleic acid synthesis. Amplification reactions include, for example, polymerase chain reactions (PCR). One PCR reaction may consist of 5 to 100 “cycles” of denaturation and synthesis of a nucleic acid molecule.

[0013] Polymerases (including DNA polymerases and RNA polymerases) useful in accordance with the present invention include, but are not limited to, Thermus thermophilus (Tth) DNA polymerase, Thermus aquaticus (Taq) DNA polymerase, Thermotoga neopolitana (Tne) DNA polymerase, Thermotoga maritima (Tma) DNA polymerase, Thermococcus litoralis (Tli or VENT™) DNA polymerase, Pyrococcus furiosus (Pfu) DNA polymerase, DEEPVENT™ DNA polymerase, Pyrococcus woosii (Pwo) DNA polymerase, Bacillus sterothermophilus (Bst) DNA polymerase, Bacillus caldophilus (Bca) DNA polymerase, Sulfolobus acidocaldarius (Sac) DNA polymerase, Thermoplasma acidophilum (Tac) DNA polymerase, Thermus flavus (Tfl/Tub) DNA polymerase, Thermus ruber (Tru) DNA polymerase, Thermus brockianus (DYNAZYME™) DNA polymerase, Methanobacterium thermoautotrophicum (Mth) DNA polymerase, mycobacterium DNA polymerase (Mtb, Mlep), and mutants, and variants and derivatives thereof. RNA polymerases such as T3, T5 and SP6 and mutants, variants and derivatives thereof may also be used in accordance with the invention.

[0014] Polymerases used in accordance with the invention may be any enzyme that can synthesize a nucleic acid molecule from a nucleic acid template, typically in the 5′ to 3′ direction. The nucleic acid polymerases used in the present invention may be mesophilic or thermophilic, and are preferably thermophilic. Preferred mesophilic DNA polymerases include T7 DNA polymerase, T5 DNA polymerase, Klenow fragment DNA polymerase, DNA polymerase III and the like. Preferred thermostable DNA polymerases that may be used in the methods of the invention include Taq, Tne, Tma, Pfu, Tfl, Tth, Stoffel fragment, VENT™ and DEEPVENT™ DNA polymerases, and mutants, variants and derivatives thereof (U.S. Pat. No. 5,436,149; U.S. Pat. No. 4,889,818; U.S. Pat. No. 4,965,188; U.S. Pat. No. 5,079,352; U.S. Pat. No. 5,614,365; U.S. Pat. No. 5,374,553; U.S. Pat. No. 5,270,179; U.S. Pat. No. 5,047,342; U.S. Pat. No. 5,512,462; WO 92/06188; WO 92/06200; WO 96/10640; Barnes, W. M., Gene 112:29-35 (1992); Lawyer, F. C., et al., PCR Meth Appl. 2:275-287 (1993); Flaman, J.-M, et al., Nucl. Acids Res. 22(15):3259-3260 (1994)). For amplification of long nucleic acid molecules (e.g., nucleic acid molecules longer than about 3-5 Kb in length), at least two DNA polymerases (one substantially lacking 3′ exonuclease activity and the other having 3′ exonuclease activity) are typically used. See U.S. Pat. No. 5,436,149; and U.S. Pat. No. 5,512,462; Barnes, W. M., Gene 112:29-35 (1992), the disclosures of which are incorporated herein in their entireties. Examples of DNA polymerases substantially lacking in 3′ exonuclease activity include, but are not limited to, Taq, Tne(exo⁻), Tma(exo⁻), Pfu(exo⁻), Pwo(exo⁻) and Tth DNA polymerases, and mutants, variants and derivatives thereof.

[0015] Host. Any prokaryotic or eukaryotic cell that is the recipient of a replicable expression vector or cloning vector. The terms “host” or “host cell” may be used interchangeably herein. For examples of such hosts, see Maniatis et al., Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y. (1982). Preferred prokaryotic hosts include, but are not limited to, bacteria of the genus Escherichia (e.g. E. coli), Bacillus, Staphylococcus, Agrobacter (e.g. A. tumefaciens), Streptomyces, Pseudomonas, Salmonella, Serratia, Caryophanon, etc. The most preferred prokaryotic host is E. coli. Bacterial hosts of particular interest in the present invention include E. coli K12, DH10B, DH5α and HB101. Preferred eukaryotic hosts include, but are not limited to, fingi, fish cells, yeast cells, plant cells and animal cells. Particularly preferred animal cells are insect cells such as Drosophila cells, Spodoptera Sf9 and Sf21 cells and Trichoplusa High-Five cells; nematode cells such as C. elegans cells; and mammalian cells such as COS cells, CHO cells, VERO cells, 293 cells, PERC6 cells, BHK cells and human cells.

[0016] Vector. A vector is a nucleic acid molecule (preferably DNA) capable of replicating autonomously in a host cell. Such vectors may also be characterized by having a small number of endonuclease restriction sites at which such sequences may be cut without loss of an essential biological function and into which nucleic acid molecules may be spliced to bring about its replication and cloning. Examples include plasmids, autonomously replicating sequences (ARS), centromeres, cosmids and phagemids. Vectors can further provide primer sites, e.g., for PCR, transcriptional and/or translational initiation and/or regulation sites, recombinational signals, replicons, etc. The vector can further contain one or more selectable markers suitable for use in the identification of cells transformed or transfected with the vector, such as kanamycin, tetracycline, amplicillin, etc.

[0017] In accordance with the invention, any vector may be used. In particular, vectors known in the art and those commercially available (and variants or derivatives thereof) may be used in accordance with the invention. Such vectors may be obtained from, for example, Vector Laboratories Inc., InVitrogen, Promega, Novagen, NEB, Clontech, Boehringer Mannheim, Pharmacia, EpiCenter, OriGenes Technologies Inc., Stratagene, Perkin Elmer, Pharmingen, Life Technologies, Inc., and Research Genetics. Such vectors may then for example be used for cloning or subcloning nucleic acid molecules of interest. General classes of vectors of particular interest include prokaryotic and/or eukaryotic cloning vectors, expression vectors, fusion vectors, two-hybrid or reverse two-hybrid vectors, shuttle vectors for use in different hosts, mutagenesis vectors, transcription vectors, vectors for receiving large inserts and the like.

[0018] Other vectors of interest include viral origin vectors (M13 vectors, bacterial phage λ vectors, baculovirus vectors, adenovirus vectors, and retrovirus vectors), high, low and adjustable copy number vectors, vectors which have compatible replicons for use in combination in a single host (pACYC184 and pBR322) and eukaryotic episomal replication vectors (pCDM8).

[0019] Particular vectors of interest include prokaryotic expression vectors such as pcDNA II, pSL301, pSE280, pSE380, pSE420, pTrcHisA, B, and C, pRSET A, B, and C (Invitrogen, Inc.), pGEMEX-1, and pGEMEX-2 (Promega, Inc.), the pET vectors (Novagen, Inc.), pTrc99A, pKK223-3, the pGEX vectors, pEZZ18, pRIT2T, and pMC1871 (Pharmacia, Inc.), pKK233-2 and pKK388-1 (Clontech, Inc.), and pProEx-HT (Life Technologies, Inc.) and variants and derivatives thereof. Vectors can also be eukaryotic expression vectors such as pFastBac, pFastBac HT, pFastBac DUAL, pSFV, and pTet-Splice (Life Technologies, Inc.), pEUK-C1, pPUR, pMAM, pMAMneo, pBI101, pBI121, pDR2, pCMVEBNA, and pYACneo (Clontech), pSVK3, pSVL, pMSG, pCH110, and pKK232-8 (Pharmacia, Inc.), p3′SS, pXT1, pSG5, pPbac, pMbac, pMC1neo, and pOG44 (Stratagene, Inc.), and pYES2, pAC360, pBlueBacHis A, B, and C, pVL1392, pBsueBacIII, pCDM8, pcDNA1, pZeoSV, pcDNA3 pREP4, pCEP4, and pEBVHis (Invitrogen, Inc.) and variants or derivatives thereof.

[0020] Other vectors of particular interest include pUC18, pUC19, pBlueScript, pSPORT, cosmids, phagemids, fosmids (pFOS1), YAC's (yeast artificial chromosomes), BAC's (bacterial artificial chromosomes), pBAC108L, pBACe3.6, pBeloBAC11 (Research Genetics), PACs, P1 (E. coli phage), pQE70, pQE60, pQE9 (Qiagen), pBS vectors, PhageScript vectors, BlueScript vectors, pNH8A, pNH16A, pNH18A, pNH46A (Stratagene), pcDNA3 (InVitrogen), pGEX, pTrsfus, pTrc99A, pET-5, pET-9, pKK223-3, pKK233-3, pDR540, pRIT5 (Pharmacia), pSPORT1, pSPORT2, pCMVSPORT2.0, pSV-SPORT1 (Life Technologies, Inc.), and the vectors described in Provisional Patent Application No. 60/065,930, filed Oct. 24, 1997, the entire contents of which is herein incorporated by reference, and variants or derivatives thereof.

[0021] Additional vectors of interest include pTrxFus, pThioHis, pLEX, pTrcHis, pTrcHis2, pRSET, pBlueBacHis2, pcDNA3.1/His, pcDNA3.1(−)/Myc-His, pSecTag, pEBVHis, pPIC9K, pPIC3.5K, pAO815, pPICZ, pPICZα, pGAPZ, pGAPZα, pBlueBac4.5, pBlueBacHis2, pMelBac, pSinRep5, pSinHis, pIND, pIND(SP1), pVgRXR, pcDNA2.1, pYES2, pZErO1.1, pZErO-2.1, pCR-Blunt, pSE280, pSE380, pSE420, pVL1392, pVL1393, pCDM8, pcDNA1.1, pcDNA1.1/Amp, pcDNA3.1, pcDNA3.1/Zeo, pSe, SV2, pRc/CMV2, pRc/RSV, pREP4, pREP7, pREP8, pREP9, pREP10, pCEP4, pEBVHis, pCR3.1, pCR2.1, pCR3.1-Uni, and pCRBac from Invitrogen; λExCell, λ gt11, pTrc99A, pKK223-3, pGEX-1λT, pGEX-2T, pGEX-2TK, pGEX-4T-1, pGEX-4T-2, pGEX-4T-3, pGEX-3X, pGEX-5X-1, pGEX-5X-2, pGEX-5X-3, pEZZ18, pRIT2T, pMC1871, pSVK3, pSVL, pMSG, pCH110, pKK32-8, pSL1180, pNEO, and pUC4K from Pharmacia; pSCREEN-1b(+), pT7Blue(R), pT7Blue-2, pCITE4abc(+), pOCUS-2, pTAg, pET-32 LIC, pET-30 LIC, pBAC-2 cp LIC, pBACgus-2 cp LIC, pT7Blue-2 LIC, pT7BIue-2, λSCREEN-1, λBlueSTAR, pET-3abcd, pET-7abc, pET9abcd, pET11abcd, pET12abc, pET-14b, pET-15b, pET-16b, pET-17b-pET-17xb, pET-19b, pET-20b(+), pET-21abcd(+), pET-22b(+), pET-23abcd(+), pET-24abcd(+), pET-25b(+), pET-26b(+), pET-27b(+), pET-28abc(+), pET-29abc(+), pET-30abc(+), pET-31b(+), pET-32abc(+), pET-33b(+), pBAC-1, pBACgus-1, pBAC4x-1, pBACgus4x-1, pBAC-3 cp, pBACgus-2 cp, pBACsurf-1, plg, Signal plg, pYX, Selecta Vecta-Neo, Selecta Vecta-Hyg, and Selecta Vecta-Gpt from Novagen; pLexA, pB42AD, pGBT9, pAS2-1, pGAD424, pACT2, pGAD GL, pGAD GH, pGAD10, pGilda, pEZM3, pEGFP, pEGFP-1, pEGFP-N, pEGFP-C, pEBFP, pGFPuv, pGFP, p6xHis-GFP, pSEAP2-Basic, pSEAP2-Contral, pSEAP2-Promoter, pSEAP2-Enhancer, pβgal-Basic, pβgal-Control, pβgal-Promoter, pβgal-Enhancer, pCMVβ, pTet-Off, pTet-On, pTK-Hyg, pRetro-Off, pRetro-On, pIRES1neo, pIRES1hyg, pLXSN, pLNCX, pLAPSN, pMAMneo, pMAMneo-CAT, pMAMneo-LUC, pPUR, pSV2neo, pYEX 4T-1/2/3, pYEX-S1, pBacPAK-His, pBacPAK8/9, pAcUW31, BacPAK6, pTrip1Ex, λgt10, λgt11, pWE15, and λTrip1Ex from Clontech; Lambda ZAP II, pBK-CMV, pBK-RSV, pBluescript II KS+/−, pBluescript II SK +/−, pAD-GAL4, pBD-GAL4 Cam, pSurfscript, Lambda FIX II, Lambda DASH, Lambda EMBL3, Lambda EMBL4, SuperCos, pWE15, pCR-Scrigt Amp, pCR-Script Cam, pCR-Script Direct, pBS +/−, pBC KS +/−, pBC SK +/−, Phagescript, pCAL-n-EK, pCAL-n, pCAL-c, pCAL-kc, pET-3abcd, pET-11abcd, pSPUTK, pESP-1, pCMVLacI, pOPRSVI/MCS, pOPI3 CAT, pXT1, pSG5, pPbac, pMbac, pMC1neo, pMC1neo Poly A, pOG44, pOG45, pFRTβGAL, pNEOβGAL, pRS403, pRS404, pRS405, pRS406, pRS413, pRS414, pRS415, and pRS416 from Stratagene, and derivatives or variants thereof.

[0022] Two-hybrid and reverse two-hybrid vectors of particular interest include pPC86, pDBLeu, pDBTrp, pPC97, p2.5, pGAD1-3, pGAD10, pACt, pACT2, pGADGL, pGADGH, pAS2-1, pGAD424, pGBT8, pGBT9, pGAD-GAL4, pLexA, pBD-GAL4, pHISi, pHISi-1, placZi, pB42AD, pDG202, pJK202, pJG4-5, pNLexA, pYESTrp and variants or derivatives thereof.

[0023] Storage. As used herein, “storage” refers to maintaining the support/vectors for a period of time at a temperature or temperatures of interest. Preferably, storage is accomplished at about 20 to 30° C. (preferably room temperature, e.g. 25° C.), but may be at higher or lower temperatures depending on the need. Lower storage temperatures may range from about 0 to 20° C., −20 to 0° C., and −80 to −20° C. Long term storage in accordance with the invention is greater than one year, preferably greater than 2 years, still more preferably greater than 3 years, still more preferably greater than 5 years, still more preferably greater than 10 years, and most preferably greater than 15 years.

[0024] Other terms used in the fields of recombinant DNA technology and molecular and cell biology as used herein will be generally understood by one of ordinary sill in the applicable arts.

[0025] It will be understood by one of ordinary skill in the relevant arts that other suitable modifications and adaptations to the methods and applications described herein are readily apparent from the description of the invention contained herein in view of information known to the ordinarily skilled artisan, and may be made without departing from the scope of the invention or any embodiment thereof. Having now described the present invention in detail, the same will be more clearly understood by reference to the following examples, which are included herewith for purposes of illustration only and are not intended to be limiting of the invention.

EXAMPLES

[0026] All reagents were from Life Technologies, Inc., Rockville, Md., unless otherwise noted.

Example 1

[0027] Preparation of Samples on an FTA™ Card. From bacterial cultures grown overnight, 5 μl were spotted in separate locations on an FTA™ Card (Cat. No. 10786) and allowed to dry overnight at room temperature. Bacterial colonies from petri dishes were spotted onto an FTA™ Card by suspending a colony in 5 μl of PBS, applying the entire volume as a single spot, then allowing the paper to dry overnight at room temperature.

[0028] For yeast genomic DNA and yeast plasmid (two-hybrid) DNAs, plates were obtained which had several colonies of each 2 two-hybrid (ProQuest, Cat. No. 10835-023) control strain. From each plate, several individual colonies were taken. Each individual colony was suspended in 5 μl PBS and each 5 μl aliquot was spotted in individual spots onto an FTA™ Card.

[0029] Using a HARRIS MICRO PUNCH™ Apparatus with mat, a 2-mm punch was taken from a dried bacterial or yeast spot (˜6 mm diameter), then washed with FTA™ Purification Reagent (Cat. No. 10876) and TE buffer according to manufacturer's recommendations. The washed punch was air dried for 1 h at room temperature or 30 min at 60° C. Processed FTA™ Card punches were either assayed immediately or stored at 4° C.

[0030] Amplification. DNA was amplified directly from a washed FTA™ Card punch placed in 50 μl of 1×PCR buffer, 1.5 mM Mg⁺⁺, 0.2 μM dNTPs, 1.25 units Platinum™ Taq DNA Polymerase, and 0.2 μM primers (Table 1). For Agrobacter tumefaciens genomic sequence, amplification was: one cycle of 94° C. for 1 min, 30 cycles of 94° C. for 1 min., 55° C. for 30 s, 72° C. for 3 min and one cycle of 72° C. for 10 min. For E coli DH10B™ genomic DNA and Streptomyces samples, amplification was: one cycle of 94° C. for 1 min, 36 cycles of 94° C. for 30 s, 55° C. for 1 min, 72° C. for 1 min, and one cycle of 72° C. for 10 min. TABLE 1 Primer sequences Amplicon Target Size (bp) Primer Sequence Agrobacter 16S rRNA 284 GGGAA AGATT TATCG GGGAT G tumefaciens GGCTG CTGGC ACGAA GTTA (SEQ ID NO:1) E. coli DH10B cells rrsE 372 CTGAG ACACG GTCCA GACTC CTACG TCACC GCTAC ACCTG GGATT CTACC (SEQ ID NO:2) AGAGT TTGAT GATCC TGGCT CAG Strepromyces 165 rRNA 1500 AAGGA GGTGA TCCAG CCGCA (SEQ ID NO:3) CCCAG TCACG ACGTT GTAAA ACG Plasmid pSUsrmB2 1503 AGCGG ATAAC AATIT CACAC AGG (SEQ ID NO:4) GAATA AGTGC GACAT CATCA TC Plasmid pMAB32 1800 GTAAA TTTCT GGCAA GGTAG AC (SEQ ID NO:5) ACTTC TTCGC CCCCG TTTTC Plasmid pJH11104 1200 GCTGA CTTGA CGGGA CGGCG (SEQ ID NO:6)

[0031] Plasmids pSUsrmB2 and pJH11104 were amplified in the same reaction mixture described above. Amplification of pMAB32 was in a reaction mixture using eLONGase™ Amplification System at 1.5 mm Mg⁺⁺. For all three plasmids, the incubation profile was one cycle of 94° C. for 1 min, one cycle of 94° C. for 15 s, and 30 cycles of 94° C. for 15 s, 55° C. for 30 s, 72° C. for 3 min.

[0032] For yeast (Saccharomyces cerevisiae) plasmid and genomic amplifications, reaction conditions using eLONGase™ Amplification System were: one cycle of 94° C. for 2 min, 40 cycles of 94° C. for 15 s, 55° C. for 20 s, 72° C. for 5 min. Primer sequences used for yeast amplification are shown in Table 2. TABLE 2 Primer sequences Amplicon Target Size (bp) Primer Sequence Plasmid pPC97 255 GAATA AGTGC GACAT CATCA TC Plasmid pPC97-RB 2088 GTAAA TTTCT GGCAA GGTAG AC (SEQ ID NO:5) Plasmid pPC97-dE2F 834 Plasmid pPC97-Fos 447 Plasmid pCL1 2853 Saccharomyces SPAL promoter 350 GCGAG GCATA TTTAT GGTGA AGG cerevisiae CATTT CCGTG CAAAG GTACT AAC MaV203(MATa) (SEQ ID NO:7)

[0033] Aliquots of each reaction product were analyzed by electrophoresis in a 1.5% (w/v) agarose/TAE gel.

[0034] Transformation. Cells were transformed with plasmid DNA from washed FTA™ Card punches, either by adding a punch directly to the reaction or by adding 5 μl of a TE buffer extract, which had soaked the punch for 20 min. at room temperature. Both MAX Efficiency DH5α™ and MAX Efficiency DH10B cells were transformed according to manufacturer's recommendations. Various dilutions of the final 1-ml transformation reaction volume (100 μl of a {fraction (1/100)} dilution, 100 μl of a {fraction (1/10)} dilution, 100 μl of undiluted cells, and 10 μl of undiluted cells) were plated on the appropriate media and incubated overnight at 37° C.

[0035] Using samples from overnight liquid cultures spotted on FTA™ Cards, Rogers and Burgoyne generated the expected diagnostic PCR patterns for each of six bacterial strains tested (Rogers, et al., (1997) Anal. Biochem. 247:223). However, according to the present invention, bacterial colonies placed on an FTA™ Card were tested. Unlike Rogers and Burgoyne who tested two complex methods of processing, all bacteria-spotted FTA™ Cards in this study were processed with simple washes.

[0036] Bacterial genomic DNA targets amplified directly from washed punches gave the expected bands (FIG. 1). FTA™ Cards were useful for screening and identifying colonies of Agrobacter bacterium from plants, a gram-negative E. coli bacterium, and a difficult-to-lyse, gram-positive Streptomyces bacterium. Success was due in part to the robust nature of the amplification reaction, not requiring quantitation of the DNA beforehand. Liquid cultures of the same bacteria spotted on the FTA™ Card may also work as well as the colonies. Also, transfer of bacteria by colony lift from the solid growth medium surface with an appropriate-sized FTA™ Card may be used. Consistent with the known properties of FTA™ Cards, bacteria could not be rescued after washed, bacteria-spotted punches were placed on solid growth media and incubated for >3 days.

[0037] Retention of plasmid DNA on FTA™ Cards was tested. Burgoyne reported that purified plasmid DNA spotted on treated paper was efficiently removed with TE buffer (after treatment with organic solvents to remove polystyrene protection coating) as measured by PCR and transformation (Burgoyne, U.S. Pat. No. 5,496,562). However, using purified DNA did not employ the advantage of directly spotting plasmid-containing-bacteria on an FTA™ Card. Three cultures of E. coli were spotted onto an FTA™ Card, and processed punches were amplified. Plasmid DNA was retained on the FTA™ Card as the expected amplicons were observed (FIG. 2). However, the amount of plasmid DNA remaining with the paper is probably low. Standard fluorescent cycle sequencing of plasmid DNA directly from a washed punch did not detect any signal (data not shown) even though plasmid DNA in a single colony has been shown to be sufficient for cycle sequencing (Young, A. and Blakesley, R. (1991) Focus 13, 137). However, sequencing of the plasmid DNA could be accomplished after the plasmid DNA was initially amplified as described above. Moreover, sequencing may be accomplished directly from the FTA™ sample under appropriate conditions which allow sufficient amounts of plasmid DNA to be retained on FTA™ paper.

[0038] Although some plasmid DNA remained with the FTA™ Card through an extensive wash procedure, it is probable the DNA is loosely associated and some of it releases during each wash. This was confirmed by generation of the correct amplicon when a 5 μl TE buffer extraction of a washed punch was amplified by PCR (data not shown). This result suggested that the released plasmid DNA from washed punches might also be recovered by biological amplification, i.e., bacterial transformation. DH5α and DH10B cells were each successfully transformed with 5 μl from a TE-buffer extraction of a washed punch previously spotted with bacteria harboring one of three plasmids (data not shown). Successful rescue of the three plasmids lead to testing a washed punch introduced directly into the cell transformation reaction (Table 3). Transformation reactions tested (two cell types and two DNA introduction methods) gave comparable results (data not shown). In all cases, bacterial clones were easily recovered, making FTA™ Cards potentially very convenient and cost effective for the long term storage of bacterial clones. Similarly, other bacterial clones harboring DNAs such as cosmids, BACs or PACs, can be recovered from samples archived on FTA™ Cards. TABLE 3 Transformation of DH5α cells with plasmids on an FTA ™ card punch Plasmid Size (kb) Copy Number Transformants/punch pSUsrmB2 5.3 6-10  7,000 pJH11104 2.7 ˜100 28,000 pMAB32 11.2 >100  5,700

Example 2

[0039] In an effort to streamline the process required to utilize FTA™ Cards for the archiving of vectors, further studies on the transformation of competent cells with plasmid DNA on FTA™ Cards were undertaken. An overnight culture of bacterial host cells (DH5α) containing the pSUsrmB2 plasmid were spotted onto FTA™ Cards. It was believed that the processing step of the FTA™ protocol could be optimized for samples that do not contain blood (examples of such samples are bacterial cells, tissue culture cells, buccal swabs, concentrates of certain body fluids such as saliva or urine, etc). The FTA™ Processing Reagent was initially designed to purify the DNA from blood samples spotted onto FTA™ Cards. This reagent is required for optimal purification of blood samples when enzyme-based assays are utilized to remove heme and other enzymatic inhibitors.

[0040] Modified processing protocols were tested for application in PCR by processing punches in a specific manner and then attempting to amplify the plasmid DNA on the punch using PCR primers (see Table 1) specific for pSUsrmB2 plasmid DNA. Punches were either not processed in any way, processed according to the manufacturer's directions using three 5 minute soaks in FTA™ Processing Reagent followed by two 5 minute soaks in TE, or processed using two abbreviated TE rinses. TE was chosen as it is a commonly used biological buffer readily available in the laboratory, although any solutions or buffer systems (e.g. PBS, TAE, TBE, Hepes, Ringers solution, Dulbecco's Phosphate buffered saline, Earle's balanced salt solution, Gey's balanced salt solution, Hank's balanced salt solution, etc., see Life Technologies catalogue) or even water may be used in this modified processing method. Preferably, solutions which do not destroy or degrade nucleic acid molecules are used. Amplification was not obtained with punches were unprocessed, but that punches receiving two brief washes with TE amplified to the same level as those processed using the full protocol. It is not unexpected that the unprocessed FTA™ punch would not produce amplification products since the reagents on the unprocessed paper would be expected to render the polymerase inactive.

[0041] The above results were obtained with standard PCR methodologies that are generally not useful for analysis of the relative amounts of DNA in any given sample. To determine if there was a difference in the amount of DNA being retained on the filter with the different processing procedures, quantitative PCR using the Perkin Elmer 7700 TaqMan machine was performed. Punch samples (2 mm) were removed from FTA™ Cards that contained spots of HeLa cells (5×10⁷ cells/ml) dried onto the paper surface. These punches were processed using either the full protocol or the abbreviated TE washes then subjected to amplification using the Perkin Elmer b-actin probe and primers in the TaqMan PCR Reagent Kit (Cat. No. N808-0230, PE Applied Biosystems, Foster City, Calif.). The signal from the FTA™ punches processed using 2 TE washes was consistently about 2-fold higher than the signal from FTA™ punches that were processed using the manufacturer's directions.

[0042] To test streamlining of the processing steps for transformation of plasmid DNA, 2 mm punches were taken from the FTA™ Cards containing overnight cultures of pSUsrmB2 and processed in different manners prior to transformation of competent DH5α cells. Punches were processed either according to the manufacturer's directions, or processed using two abbreviated rinses of TE, or used unprocessed, directly from the FTA™ Cards. The results in Table 4 show that the 2 TE washes produce the maximum number of colonies per punch but that an unprocessed punch also produces sufficient numbers of colonies for archival purposes. The lowest number of colonies was obtained using the full manufacturer's processing protocol, again indicating that DNA was being removed from the punch with the additional washing steps. Additional studies have shown that a punch washed just once in TE gives slightly more colonies than an unprocessed punch and slightly less than a punch washed twice in TE, additional TE washes over two decreases the number of colonies obtained. While DNA amplification could not occur with an unprocessed punch, plasmid transformation can, although not as efficiently as with a minimally processed punch. This slight loss of efficiency can be explained by the loss in viability of some of the competent cells in a reaction with an unprocessed punch. TABLE 4 Punch Processing Protocol Total Colonies per 2 mm Punch* unprocessed 137 TE washes 193 full processing 45

Example 3

[0043] To show the utility of FTA™ over other similar collection devices for the archiving of plasmid DNA, an overnight culture of bacterial host cells (DH5α) containing the pSUsrmB2 plasmid were spotted onto FTA™ cards or similar paper-based collection devices and allowed to air-dry. The other collection devices used were: Isocode PCR DNA Sample Collection Device (Schleicher & Schuell, Keene, N.H.), Generation Capture Card Kit (Gentra Systems, Minneapolis, Minn.) and Whatman # 4 filter paper (Clifton, N.J.). Whatman # 4 filter paper has been used historically by researchers for short-term storage of live bacterial cells for applications such as transfer of a strain of bacteria between laboratories by mail or delivery service. Live bacterial cells can be recovered from the filter paper by placing a portion of the filter paper into a suitable culture medium for growth.

[0044] Punches (2 mm) were taken from each of these collection devices and the FTA™, Isocode and Generation products were processed according to the manufacturer's directions and with the two abbreviated TE washes described above. The Isocode product is designed to release DNA from the paper, therefore both the processed punch as well as a one-tenth volume (5 ml) of the released DNA were tested. The Whatman # 4 filter paper punches were not processed in any manner. The punches were then used in a transformation experiment using DH5α competent cells. In addition, a TE washed punch (or in the case of the Whatman # 4 filter paper, an unprocessed punch) was placed into a control mock transformation containing 100 ml of SOC medium instead of 100 ml of competent cells to test that all the colonies obtained in the transformation experiments were derived from actual transformation events and not from carry-over of live bacteria.

[0045] The results in Table 5 show that the Gentra Generations product does not produce numbers of transformants in the same range as FTA™ paper. The Isocode product produced numbers of colonies in the same range as FTA™ paper, but only when the paper is processed first. The total number of colonies obtained will be influenced by copy number and size of the plasmid insert used. As expected, the Whatman # 4 paper was an effective method for short-term storage of culturable bacterial cells shown by the equal numbers generated with and without competent cells, but not for long-term recovery of cells. Due to the nature of FTA™ Cards, the DNA stored on FTA™ paper is likely to be protected from damage for the long-term. Bacterial cells on FTA™ paper have shown no loss in transformation efficiency for at least 3 months. Blood stored on FTA™ paper for more than 7 years has yielded DNA for PCR analysis. TABLE 5 Total Number of Colonies per 2 mm Punch (pSUsrmB2 culture) Gentra S&S Whatman Whatman Processing Genera- Iso- #4 #4 Method FTA ™* tion* code (10 days) (25 days) un- 137 2 5 247 0 processed 2TE 193 5 170 N.D. N.D. manu- 45 0 15 N.D. N.D. facturer's protocol released N.D. N.D. 40 N.D. N.D. DNA mock 0 0 0 263 10 transfection

Example 4

[0046] Additional studies on the utility of FTA™ paper with the M13 vector system were undertaken. M13 is a bacteriophage vector system that has the ability to produce single stranded DNA molecules that are particularly useful as DNA sequencing templates. However, preparation of purified templates is tedious and time-consuming. FTA™ Cards were tested to see if they could simplify the purification of the sequencing template DNA. M13 plaques were either directly transferred to FTA™ paper or host DH5αFIQ cells infected with M13 were applied to FTA™ paper and allowed to dry. Punches (2 mm) were taken from the FTA™ Cards and processed with TE (as these samples do not contain blood). After processing, the punches were subjected to fluorescent automated sequencing using the ABI Prism Big Dye Terminator Cycle Sequencing Ready Reaction Kit (Cat. No. 4303149, PE Applied Biosystems, Foster City, Calif.) according to the manufacturer's directions and the resulting reactions were analyzed on the ABI Prism 377.

[0047] An excellent sequence was obtained from the M13 plaque that was directly transferred to the FTA™ Card. The read-length was greater than 600 nucleotides with no unreadable bases in the first 600 bases. When this sequence was compared to the known sequence of M13, there were 0 errors in the first 300 nucleotides and one error and one misread in the next 300 nucleotides (error rate 0.33% for 600 nucleotides). Sequence data generated from M13 infected cells on FTA™ was readable, but less error-free indicating that sequence information can be obtained from this format, but optimization of cell concentration or processing methods may be required. M13 plaques placed directly on either Gentra Generations cards or Isocode cards also produced readable sequences.

[0048] The FTA™ Card is known for its utility in archiving, its ease of sample preparation, and elimination of potential biohazards in DNA from blood samples. According to the present invention, any matrix or solid medium (preferably a cellulose or paper based matrix and particularly FTA™ Cards) are also useful for archiving DNA from bacterial sources, both genomic and vectors. Thus, the invention represents a method for convenient and efficient storage, processing and recovery of vector or plasmid clones. This method could be very useful in storage of the vast numbers of subclones generated, for example, in large-scale genome sequencing projects.

[0049] Having now fully described the present invention in some detail by way of illustration and example for purposes of clarity of understanding, it will be obvious to one of ordinary skill in the art that the same can be performed by modifying or changing the invention within a wide and equivalent range of conditions, formulations and other parameters without affecting the scope of the invention or any specific embodiment thereof, and that such modifications or changes are intended to be encompassed within the scope of the appended claims.

[0050] All publications, patents and patent applications mentioned in this specification are indicative of the level of skill of those skilled in the art to which this invention pertains, and are herein incorporated by reference to the same extent as if each individual publication, patent or patent application was specifically and individually indicated to be incorporated by reference.

1 7 1 40 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 1 gggaaagatt tatcggggat gggctgctgg cacgaagtta 40 2 50 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 2 ctgagacacg gtccagactc ctacgtcacc gctacacctg ggattctacc 50 3 43 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 3 agagtttgat gatcctggct cagaaggagg tgatccagcc gca 43 4 46 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 4 cccagtcacg acgttgtaaa acgagcggat aacaatttca cacagg 46 5 44 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 5 gaataagtgc gacatcatca tcgtaaattt ctggcaaggt agac 44 6 40 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 6 acttcttcgc ccccgttttc gctgacttga cgggacggcg 40 7 46 DNA Artificial Sequence Description of Artificial Sequence synthetic oligonucleotides 7 gcgaggcata tttatggtga aggcatttcc gtgcaaaggt actaac 46 

What is claimed is:
 1. A composition comprising: a) a cellulose based solid matrix or a micromesh synthetic plastic matrix; and b) one or more vectors, wherein said matrix is not coated or encased with polystyrene.
 2. The composition according to claim 1, wherein said matrix comprises a composition comprising a weak base, a chelating agent, an anionic surfactant or anionic detergent, and optionally uric acid or a urate salt, wherein said composition is adsorbed on or incorporated into said solid matrix.
 3. The composition according to claim 1, wherein said matrix is not coated or encased with a protective coating.
 4. The composition according to claim 1, wherein said matrix is FTA™ paper or derivatives, variants or modifications thereof.
 5. The composition of claim 1, further comprising one or more polymerases.
 6. The composition of claim 5, wherein said polymerases are DNA polymerases.
 7. The composition of claim 6, wherein said DNA polymerases are thermostable DNA polymerases.
 8. The composition of claim 1, further comprising one or more host cells.
 9. The composition of claim 8, wherein said host cells are chemically competent or electrocompetent.
 10. The composition of claim 1, further comprising one or more components selected from the group consisting of one or more primers, one or more polymerases and one or more nucleotides.
 11. A method for storage of one or more vectors comprising: a) contacting said vectors with a cellulose based solid matrix or a micromesh synthetic plastic matrix; and b) storing said vectors contacted with said matrix, wherein said matrix is not coated or encased with polystyrene.
 12. The method according to claim 11, wherein said matrix comprises a composition comprising a weak base, a chelating agent, an anionic surfactant or an anionic detergent and optionally uric acid or a urate salt.
 13. The method of claim 11, wherein said contacting is accomplished under conditions sufficient to associate said vectors with said matrix.
 14. The method of claim 11, further comprising purifying or isolating said vectors from said matrix.
 15. The method according to claim 11, further comprising removing said vectors from said matrix for subsequent treatment.
 16. The method according to claim 15, wherein said treatment is selected from the group consisting of digestion, synthesis, amplification, sequencing, transformation or transfection of said vectors.
 17. The method according to claim 11, further comprising treating or manipulating said vectors.
 18. The method according to claim 17, wherein said treatment or manipulation is selected from the group consisting of digestion, synthesis, amplification, sequencing, transformation or transfection of said vectors.
 19. The method according to claim 18, wherein said treatment is amplification by polymerase chain reaction.
 20. The method of claim 18, wherein said treatment is transformation or transfection.
 21. The method of claim 20, wherein said vectors are transformed into a prokaryotic host.
 22. The method of claim 21, wherein said prokaryotic host is E. coli.
 23. The method of claim 18, wherein said digestion is digestion with a restriction endonuclease.
 24. The method of claim 18, wherein said amplification is accomplished with a polymerase.
 25. The method of claim 24, wherein said polymerase is Taq DNA polymerase or a mutant, variant or derivative thereof.
 26. A method of isolating or purifying one or more vectors comprising: a) contacting a matrix or solid medium with a sample containing said vectors; and b) isolating all or a portion of said vectors from said medium.
 27. The method of claim 26, wherein said medium protects against degradation of said vectors.
 28. The method of claim 26, wherein said sample is selected from the group consisting of host cells, viruses, extracts of host cells or viruses, lysates of host cells or viruses, host cell or virus debri, and combinations thereof.
 29. A method for treating or manipulating one or more vectors comprising: a) contacting a sample containing said vectors with a solid medium or matrix; and b) treating or manipulating all or a portion of said vectors.
 30. The method of claim 29, wherein said sample is selected from the group consisting of host cells, viruses, extracts of host cells or viruses, lysates of host cells or viruses, host cell or virus debri, and combinations thereof.
 31. The method of claim 29, wherein said matrix or medium in FTA™ paper or derivatives, variants or modifications thereof.
 32. The method of claim 29, wherein said treatment or manipulation is selected from the group consisting of digestion, synthesis, amplification, sequencing, transformation or transfection. 